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www.sciencemag.org/content/344/6187/992/suppl/DC1
Supplementary Materials for
Crystal structure of a heterotetrameric NMDA receptor ion channel
Erkan Karakas and Hiro Furukawa*
*Corresponding author. E-mail: furukawa@cshl.edu
Published 30 May 2014, Science 344, 992 (2014) DOI: 10.1126/science.1251915
This PDF file includes
Materials and Methods Figs. S1 to S16 Table S1 References
2
Materials and Methods
Construct Design
The genes encoding the C-terminally truncated rat GluN1a (residues 1-847,
accession code: P35439) and GluN2B (residues 27-852, accession code: Q00960), which
is C-terminally truncated and N-terminally fused to GluN1 signal peptide, OneStrep tag
and a thrombin recognition site, were cloned into pUCDM and pFL vectors, respectively
(40). Polyhedrin promoter in the original vectors was replaced by Hsp70 promoter. Those
two plasmids were recombined using Cre recombinase as described previously (40). To
improve crystal quality of GluN1a/GluN2B NMDA receptors, the following mutations
were initially incorporated: 1) 6 out of 11 putative glycosylation sites on GluN1a and 1
out of 6 putative glycosylation sites on GluN2B were removed by mutations on GluN1a
(Asn61Gln, Asn239Asp, Asn350Gln, Asn471Gln, Asn491Gln and Asn771Gln) and on
GluN2B (Asn348Asp); 2) cysteine residues, Cys22 on GluN1a and Cys588, Cys838 and
Cys849 on GluN2B were mutated to serine to avoid non-specific disulfide bond
formation; 3) six residues, Cys395, Pro396, Glu397, Glu399, Glu400 and Glu402, were
removed from the ATD-LBD linker on GluN2B; and 4) patches of charged residues on
the cytoplasmic loop of GluN1a was neutralized by mutations, Glu594Gln, Glu595Ser,
Glu597Ser, Glu598Thr, Arg844Asn, Arg845Gly and Lys846Ala. This construct,
GluN1a/GluN2Bcryst, crystallized and resulted in 5.7 Å resolution structure. Based on the
structure, GluN1a/GluN2Bcrystx construct was designed and made by introducing the
GluN2B Ser214Cys mutation to cross-link the two GluN2B ATDs and GluN1a-
Thr561Cys/GluN2B-Ile815Cys and GluN1a-Phe810Cys/GluN2B-Asp557Cys mutation
pairs at the TMD to further stabilize the heterotetramer.
Expression and purification
Large scale expression of GluN1a/GluN2Bcrystx NMDA receptors were performed by
infecting Sf9 insect cells at a cell density of 4 x 106 cells/ml using baculovirus harboring
both GluN1acrystx and GluN2Bcrystx genes under the control of HSP70 promoter from
Drosophila melanogaster. At 48 hours post infection, cells were harvested by
centrifugation at 1,000 g for 20 min. and lysed in a buffer composed of 150 mM NaCl, 20
mM HEPES-NaOH pH 7.3 and 1 mM phenylmethylsulphonyl fluoride (PMSF) using
Avestin EmulsiFlex-C5. The cell lysate was centrifuged at 6,000 g for 25 minutes and the
membrane was pelleted by centrifugation at 185,000 g for 1 hour. The membranes were
homogenized and solubilized in 180 mM NaCl, 40 mM HEPES-NaOH pH 7.3 and 0.5%
lauryl maltose neopentyl glycol (MNG-3) for 3 hours, prior to centrifugation at 185,000 g
for 40 minutes to remove insoluble materials. The GluN1a/GluN2Bcrystx proteins in the
supernatant were loaded onto Strep-tactin Superflow, washed with 15 column volumes of
the wash buffer composed of 500 mM NaCl, 20 mM HEPES-NaOH pH 7.3, 0.01%
MNG-3 and 0.01 mg/ml 1-palmitoyl-2-oleoyl-sn-glycero-3-phosphocholine (POPC), and
eluted with the same buffer containing 3 mM d-desthiobiotin. Following thrombin
digestion to remove the strep tag at 18°C overnight, protein was further purified by size
exclusion chromatography using Superose 6 (10/300 GL, GE Healthcare) equilibrated
with 200 mM NaCl, 20 mM HEPES-NaOH pH 7.3, 0.01% MNG-3 and 0.01 mg/ml
POPC at room temperature. The fractions that correspond to GluN1a/GluN2Bcrystx were
concentrated to 4.5-5 mg/ml, supplemented with 10 mM glycine, 10 mM L-glutamate
3
and 0.1 mM ifenprodil and used for crystallization immediately. To produce SeMet-
incorporated GluN1a/GluN2Bcrystx proteins, the culture medium was substituted with
methionine free ESF921 media prior to viral infection. After one hour, L-SeMet at 75
mg/L was added to the culture and the media was harvested 48 h post infection. The
proteins were purified as described above.
Crystallization
Crystals of GluN1a/GluN2Bcryst NMDA receptors were initially obtained by vapor
diffusion using a reservoir solution of 15% PEG 4000, 0.1 M Tris-HCl (pH 8.5) and 0.2
M MgCl2 (MembFac, Hampton Research). However, the diffraction was limited to 8.0 Å
after extensive optimization of the crystallization conditions. Use of Mg(OAc)2 instead of
MgCl2 dramatically increased crystal size by 3 fold and increased the diffraction power to
~7.0 Å. Diffraction power was further improved by including synthetic lipids, POPC, in
purification buffers and incubating crystals in 1 M Mg(OAc)2 containing buffer, which
also acted as cryo-protectant, for 24 hours prior to flash freezing. The most dramatic
improvement was observed on crystals soaked with the heavy atom cluster, hexa-sodium
metatungstate, where diffraction reached up to 5.7 Å. At this point, we were able to
obtain a structure of GluN1a/GluN2Bcryst NMDA receptor by molecular replacement as
described below. This low resolution structure was used to design cross-linking mutations
to stabilize the tetramer. After extensive screening of cross-link constructs for
crystallization and x-ray diffraction, the GluN1a/GluN2Bcrystx (described above) yielded
crystals that diffracted beyond 4.0 Å. The best diffracting crystals of
GluN1a/GluN2Bcrystx NMDA receptor were obtained by vapor diffusion at 18 °C in
hanging drops containing 1.4 µl of protein solution, 0.5 µl of reservoir solution (10-12%
PEG 4000, 0.2 M NaCl, 0.1 M Tris-HCl pH 8.8 and 0.4 M Mg(OAc)2), and 0.4 µl of 0.1
mM hexa-sodium metatungstate. Crystals were first incubated in a buffer containing 12%
PEG 4000, 0.08 M Tris-HCl pH 8.8, 0.02 M HEPES-NaOH pH 7.3, 0.2 M NaCl, 1 M
Mg(OAc)2, 0.01% MNG-3, 10 mM glycine, 10 mM L-glutamate, 0.1 mM ifenprodil,
0.01 mg/ml POPC, and 0.05 mM hexa-sodium metatungstate for 24 hours and flash
frozen by liquid nitrogen after soaking in the same buffer but with higher hexa-sodium
metatungstate concentration (1 mM) for 2 hours. Holmium and gadolinium derivatives
were obtained by including 100 mM HoCl3 or GdCl3 in the final soaking buffer.
Data collection and structure determination
Data collection was performed using synchrotron radiation at the beamlines ID23-B
and ID23-D at the Advanced Photon Source (APS) at Argonne National Laboratory and
at the beamline BL41XU at SPring-8. Datasets were indexed, integrated and scaled using
HKL2000 (41). Diffraction power of the datasets collected from single crystals was
limited to 4.2 Å due to radiation damage. Therefore, datasets collected from 15 different
crystals of GluN1a/GluN2Bcrystx construct were indexed and integrated separately and
scaled together using HKL2000 (41). The structure was solved by molecular replacement
using the coordinates of GluN1b/GluN2B ATD (PDB code: 3QEL) (7) and
GluN1/GluN2B LBD model built based on the GluN1/GluN2A LBD structure (PDB
code: 2A5T) (12) with the program PHASER (42). The model was built using COOT
(43) and initial structural refinement was performed using jellybody refinement
implemented in the program REFMAC (17) along with PROSMART (44) to create
4
restraints based on the high resolution structures of the isolated ATD and LBD structures
and using deformable elastic network (DEN) refinement (18). Final refinement cycles
were performed using Phenix (45) with restraints based on two-fold non-crystallographic
symmetry, secondary structure and high resolution structures of ATD and LBDs.
Cysteine cross-linking and western blot
Proteins with incorporated cysteine mutations on GluN1a/GluN2Bcryst constructs
were expressed as described above. Harvested cell pellets were solubilized in a buffer
composed of 150 mM NaCl, 20 mM HEPES-NaOH pH 7.3, 0.5% MNG-3, 10 mM
glycine, 10 mM L-glutamate, 0.01 mM ifenprodil and 1mM PMSF and centrifuged at
185,000g. The GluN1a/GluN2B proteins in the supernatant were purified using Strep-
tactin Superflow resin and subjected to SDS-polyacrylamide gel electrophoresis (7%) in
the presence and absence of 150 mM β-mercaptoethanol. The proteins were transferred to
Hybond-ECL nitrocellulose membranes (GE Healthcare). The membrane was blocked
with 5% milk in TBST (20 mM Tris-HCl pH 8.0, 150 mM NaCl and 0.05% Tween-20),
then incubated with mouse monoclonal antibodies against GluN1 (MAB1586, Millipore)
or GluN2B (ab93610, Abcam), followed by HRP-conjugated anti-mouse antibodies (GE
Healthcare). Protein bands were detected by ECL detection kit (GE Healthcare).
Electrophysiology
Recombinant GluN1a/GluN2B NMDA receptors were expressed by co-injecting
0.1-0.5 ng of the wild-type or mutant rat GluN1a and GluN2B cRNAs at a 1:2 ratio (w/w)
into defolliculated Xenopus laevis oocytes. The two-electrode voltage-clamp recordings
were performed using agarose-tipped microelectrodes (0.4-1.0 MΩ) filled with 3 M KCl
at a holding potential of -60 mV. The bath solution contained 5 mM HEPES, 100 mM
NaCl, 0.3 mM BaCl2 and 10 mM Tricine at pH 7.4 (adjusted with KOH). Currents were
evoked by applications of 100 μM of glycine and L-glutamate and potentiated or
allosterically inhibited by spermine and ifenprodil, respectively. Whole-cell patch-clamp
recordings were performed on HEK 293 cells transfected with GluN1acryst in pUCDM
and GluN2Bcryst in pFL under CMV promoter. All of the recordings were done at −60 mV
(23 °C) with micropipettes containing (in mM) 110 D-gluconate, 110 CsOH, 30 CsCl, 5
HEPES, 4 NaCl, 0.5 CaCl2, 2 MgCl2, 5 BAPTA, 2 NaATP and 0.3 NaGTP (pH 7.35).
The external solution contained (in mM) 150 NaCl, 10 HEPES, 30 D-mannitol, 3 KCl,
1.0 CaCl2 and 0.01 EDTA at 23°C and pH 7.4. Rapid solution exchange was
accomplished with a piezoelectric driven two barreled theta glass pipette (Burleigh
Instruments, Newton NJ); typical 10-90% exchange times for solutions around the cells
were < 3ms. Deactivation and desensitization time course were fitted with the double
exponential equation: Response = AmplitudeFAST (exp(-time/tauFAST)) +
AmplitudeSLOW(exp(-time/tauSLOW). Data acquisition was performed with pClamp version
9-10 and analysis performed using Channelab.
5
Fig. S1. Construct design of NMDA receptor subunits. Schematic representation
of rat GluN1acrystx (yellow) and GluN2Bcrystx (cyan) subunits highlighting the
modification performed on both constructs. Amino terminal domain (ATD), ligand
binding domain (LBD), transmembrane domain (TMD) and carboxy terminal domain
(CTD) for both subunits are shown as separate domains. The GluN1a subunit is truncated
at the C-terminus (Gln 847) and expressed with the native signal peptide. C-terminally
truncated GluN2B subunit is fused to the signal peptide from GluN1a, OneStrep tag, and
a thrombin recognition site at the N-terminus (Arg 27). Mutations to remove predicted
glycosylation sites are highlighted in green. Cysteine to serine mutations to avoid non-
specific disulfide bond formation are shown in orange and residues that are removed
from the ATD and LBD linker on GluN2B subunits are shown in blue. Point mutations to
neutralize the charged groups of residues at the cytoplasmic side of GluN1a subunit are
indicated in red. To stabilize the tetrameric arrangement of the NMDA receptor, cysteine
mutations (purple) are introduced to cross-link M1 helices to the M4 helices of the
neighboring subunits at the TMD and the two GluN2B ATDs.
6
Fig. S2: Expression and purification of GluN1a/GluN2B NMDA receptors. (A)
GluN1acryst that is fused to EGFP at the C-terminal end is co-expressed with GluN2Bcryst
in Sf9 insect cells under heat-shock protein promoter from Drosophila melanogaster (red,
dHSP) or polyhedrin promoter (blue, polH) using baculovirus. The GluN1acryst-
EGFP/GluN2Bcryst NMDA receptor proteins are extracted by MNG-3 and detected by
fluorescence coupled size exclusion chromatography (FSEC) (475 nm excitation/507 nm
emission) (46). The major peak at the retention time of ~2,000 second for the sample
expressed under dHSP represents heterotetramers. Such peak is almost absent when the
proteins are expressed under polH. (B) Purification of GluN1a/GluN2Bcrystx NMDA
receptor proteins from insect cells using Strep-tactin Superflow. SDS-PAGE showing
MNG-3 solubilized material (lane 1), flow through fraction from the column (lane 2), the
elution fraction (lane 3), and the elution fraction treated with thrombin to remove
OneStrep tag fused to GluN2Bcrystx (lane 4). (C) Size exclusion chromatogram of purified
GluN1a/GluN2Bcrystx NMDA receptor proteins detected by intrinsic tryptophan
fluorescence (280 nm excitation/330 nm emission).
8
Fig. S3: Multiple sequence alignment of GluN1acrystx with other ionotropic
glutamate receptor subunits. Shown here are the primary sequences of GluN1acrystx, rat
GluN1a (P35439), rat GluN2B (Q00960), rat GluA2i (NP_058957) and GluK1
(P22756_2). Sequences for the C-terminal domain are excluded from the alignment. The
sequence alignment is annotated with arrows for β-strands, cylinders for α- and η (310)-
helices and lines for loops based on the crystal structure of GluN1acrystx. The structural
annotation is colored according to domains as magenta (ATD), orange (LBD) and cyan
(TMD). Disordered regions with no clear electron density are shown as dashed lines. The
names of the helices and strands are kept the same as in high resolution structures of
isolated GluN1b/GluN2B ATD (α, η and β prefixed) and GluN1/GluN2A LBD (capital
letters and numbers). Mutated residues are highlighted with the same color code as in Fig.
S1.
10
Fig. S4: Multiple sequence alignment of GluN2Bcrystx with ionotropic glutamate
receptors. Shown here are the primary sequences of GluN2Bcrystx, rat GluN2B (Q00960),
rat GluN1a (P35439), rat GluA2i (NP_058957) and GluK1 (P22756_2). Sequences for
the C-terminal domain are excluded from the alignment. The sequence alignment is
annotated with arrows for β-strands, cylinders for α- and η (310)-helices and lines for
loops based on the crystal structure of GluN2Bcrystx. The structural annotation is colored
according to domains as magenta (ATD), orange (LBD) and cyan (TMD). Disordered
regions with no clear electron density are shown as dashed lines. The names of the
helices and strands are kept the same as in high resolution structures of isolated
GluN1b/GluN2B ATD (α, η and β prefixed) and GluN1/GluN2A LBD (capital letters and
numbers). Mutated residues are highlighted with the same color code as in Fig. S1.
11
Fig. S5: Electrophysiological measurement of the response time course of
mutant GluN1a/GluN2B NMDA receptors. (A-D) Representative whole cell patch-
clamp recordings of wild-type GluN1a/GluN2B (A and C) and GluN1a/GluN2Bcryst (B
and D) expressed in HEK293 cells and activated with long (A and B; 1.5 sec) and brief
(C and D; 5 msec) application of 1 mM glutamate in the constant presence of 100 µM
glycine. The cells were voltage-clamped at −60 mV. (E-G) Comparison of time courses
for activation (E), desensitization (F), and deactivation (G) of wild-type GluN1a/GluN2B
and GluN1a/GluN2Bcryst.
12
Fig. S6: Electrophysiological properties of GluN1a/GluN2B NMDA receptor
mutants. (A and B) Allosteric inhibition of the wild-type (A) and GluN1a/GluN2Bcryst
(B) NMDA receptors by two different concentrations of ifenprodil (IF). Glut represents
100 µM of L-glutamate. (C and D) Potentiation of Glut-induced currents in the wild-type
(C) and GluN1a/GluN2Bcryst (D) NMDA receptors by spermine (100 µM). The patterns
of both ifenprodil mediated allosteric inhibition and spermine mediated potentiation are
similar between the wild-type and GluN1a/GluN2Bcryst NMDA receptors indicating the
physiological relevance of the mutant construct. (E to H) Redox experiments using two-
electrode voltage clamp on Xenopus oocytes injected with cRNAs for
GluN1a/GluN2Bcryst NMDA receptors (E), GluN1a/GluN2Bcryst (Ser214Cys) NMDA
receptors (F), GluN1acryst-Thr561Cys-Phe810Cys/GluN2Bcryst-Asp557Cys-Ile815Cys
(G), and GluN1a/GluN2Bcrystx NMDA receptors (equivalent to GluN1acryst Thr561Cys-
Phe810Cys/GluN2Bcryst Ser214Cys-Ile815Cys-Asp557Cys) (H). There is little or no
change upon addition of 2 mM of DTT in GluN1a/GluN2Bcryst NMDA receptors whereas
the major potentiation in GluN1a/GluN2Bcryst (Ser214Cys) and GluN1a/GluN2Bcrystx
NMDA receptor is observed. The current for GluN1a/GluN2Bcrystx NMDA receptor is
typically small compared to that for GluN1a/GluN2Bcryst NMDA receptors likely caused
by inefficient surface expression in Xenopus oocytes. (I-K) The redox experiment done
by whole-cell patch clamp on HEK293 cells expressing GluN1a/GluN2Bcryst (Ser214Cys)
NMDA receptors (I), GluN1a-Thr561Cys-Phe810Cys/GluN2Bcryst-Ile815Cys-
Asp557Cys (J), and GluN1a/GluN2Bcrystx NMDA receptors (K). In all of the cases, wash
buffer contained 100 µM of glycine.
13
Fig. S7: Electron density maps of GluN1a/GluN2Bcryst (non-cross-linked). (A) 2FoFc map calculated using the 5.7 Å x-ray diffraction data from the GluN1a/GluN2Bcryst
crystal is contoured at 1 σ and shown as grey mesh over the Cα trace of
GluN1a/GluN2Bcrystx structure. Electron density clearly shows that incorporation of
cross-linking mutations did not cause a major change in overall GluN1a/GluN2B
structure. (B) The close up view of the TMD from panel A.
14
Fig. S8: Electron densities in the transmembrane domains in
GluN1a/GluN2Bcrystx. 2FoFc maps for the M1, M2, M3 and M4 helices of both GluN1a
(α) and GluN2B (β) TMDs are prepared with a B-factor sharpening factor of -90 Å2,
countered at 1.0 σ and shown as grey mesh. The models of GluN1a (α) and GluN2B (β)
are shown as yellow and cyan Cα traces, respectively. Cαs of methionine residues are
shown as spheres. Anomalous difference Fourier maps calculated from data collected on
two different selenomethionine-derivative crystals are averaged around the 2-fold non-
crystallographic axis using COOT (43) and shown as red mesh. The maps are contoured
at the following σ levels; 2.8 σ for GluN1a Met 555, 3.6 σ for GluN1a Met 576, 2.5 σ for
GluN1a Met 607, 2.5 σ for GluN1a Met 634, 4.2 σ for GluN1a Met 641, 3.3 σ for
GluN1a Met 813, 2.7 σ for GluN1a Met 818, 2.5 σ for GluN2B Met 561, 2.8 σ for
GluN2B Met 631, 2.5 σ for GluN2B Met 654, 3.0 σ for GluN2B Met 824 and 2.5 σ for
GluN2B Met 829. No significant signal was observed for residues GluN2B Met 562 and
Met 565.
15
Fig. S9: Electron density maps for the ligands. FoFc electron density maps for the
three ligands, ifenprodil (A), glycine (B) and L-glutamate (C) at their respective binding
sites are shown as green mesh and contoured at 4, 3 and 3 σ levels, respectively. Ligands
are shown as light grey sticks.
16
Fig. S10: Electron density maps for GluN1a/GluN2Bcrystx. 2FoFc electron density
maps for GluN1acrystx (left) and GluN2Bcrystx (right) subunits are show as grey mesh and
countered at 1 σ. Maps are sharpened by a B factor of -90 Å2. Cα traces for GluN1a (left)
and GluN2B (right) subunits are shown. Note the distal and proximal positioning of the
ATD-LBD linkers for GluN1a and GluN2B, respectively, as pointed with arrows.
17
Fig. S11: Dimer-of-dimers assembly of GluN1a/GluN2B NMDA receptors.
Tetrameric arrangement of ATD (A), LBD (B) and TMD (C) of GluN1a/GluN2Bcrystx
NMDA receptors viewed from top (left panels) and side (right panels). Regions at the
dimer-of-dimers interfaces are highlighted and residues in close proximity at ATD and
LBD are shown as sticks on the side view. Side view of LBD (panel B, right) is one
(between GluN1a (α) and GluN2B (α)) of the two equivalent sites of dimer-of-dimers
interaction at LBD.
18
Fig. S12: Probing inter-subunit interfaces in GluN1a/GluN2B NMDA
receptors. (A) Western blot analysis of spontaneous disulfide cross-linking of cysteine
substituted GluN1a/GluN2Bcryst NMDA receptors probed by anti-GluN1 (top) and anti-
GluN2B (bottom) antibodies under reducing conditions. (B) Western blot analysis of
wild-type (wt) GluN1acryst / cysteine substituted GluN2Bcryst and cysteine substituted
GluN1acryst / wt GluN2Bcryst NMDA receptors probed by anti-GluN1 (top) and anti-
GluN2B (bottom) antibodies under non-reducing conditions. Arrows indicate positions of
the monomers.
19
Fig. S13: Assessing various patterns of subunit arrangements at LBD. (A and B)
Arrangement of GluN1a (β) and GluN2B (β) in the 1-2-1-2 arrangement observed in the
crystal structure. (C) Swapping GluN1a and GluN2B to make 2-1-2-1 arrangement
results in the clashes between GluN1a Loop 1 and GluN2B Helix G’ and between
GluN1a Helix K and GluN2B Helix E’ and F’ (dashed circles). (D and E) Superposition
of GluN1a onto GluN2B (D) or GluN2B onto GluN1a (E) to enforce 1-1-2-2
arrangement causes clashes between GluN1a Loop 1 and GluN1a Helix G and between
GluN2B Helix E’, F’ and K’ (dashed circles).
20
Fig. S14: Functionally critical elements located at the dimer interface of the
GluN1a/GluN2B heterodimers. The critical sites at the extracellular region (GluN1a
Asp 669 and GluN2B Ser214Cys’ and Loop 1’) where mutations have significant
implication in function are highlighted and labeled on the overall structure of
GluN1a/GluN2B NMDA receptors.
21
Fig. S15: Plausible changes in ATD conformation move the location of LBDs.
(A-B). We make an assumption that the bilobed structures of ATD twist and untwist
between the two lobes, R1 and R2, as previously reported (28). Untwisting of GluN1a
(A) and GluN2B (B) by ~40o is accomplished by rotating R2 (lower lobe tethered directly
22
to LBD) using GluK1 ATD structure (30) as a guide. (C to F) Shown here are structures
of ATD tetramers viewed “up” from the LBDs. The ATDs in the current crystal structure
and the previously published GluN1b/GluN2B ATD structures have “twisted”
conformations in both GluN1 and GluN2B (C). Untwisting of GluN1a (D), GluN2B (E),
or both (F) dramatically changes the location of LBDs. Numbers next to the dashed lines
represent distance (in Å) between the beginning points of LBD defined as the Cαs of
GluN1a Thr396 and GluN2B His405 (spheres). Note that untwisting of both GluN1a and
GluN2B ATDs result in separation of the LBDs in both length and width to significantly
more extent in GluN1a than GluN2B. This separation likely results in rearrangement of
subunits within and between the GluN1a/GluN2B LBD thereby affecting patterns of ion
channel gating. Shown in gray spheres are GluN2B Ser214 residues from both GluN2B
(α) and (β). Formation of a disulfide bond by the GluN2B Ser214Cys mutation at the
lower lobe (R2) not only traps the inter-subunit arrangement between the two GluN2B
subunits, but also movement in the GluN2B ATD lobes.
23
Fig. S16: Structural comparison of NMDA receptor ion channel with potassium
channels. TMDs of GluN1a subunits (yellow, left panel) and GluN2B subunits (cyan,
middle panel) are superposed onto the ion channel domains (red) of the closed
conformation of KcsA (PDB ID: 1K4C) (A), open conformation of MthK (PDB ID:
3LDC) (B). The superposed structures are viewed from the side (left and middle panels)
or from the extracellular side (right panel). Superposition is performed using Secondary-
structure matching (SSM) tool. Loops are excluded from the figure for clarity.
24
Table S1. Data collection and refinement statistics
GluN1a/
GluN2B
cryst
GluN1a/
GluN2B
crystx
GluN1a/
GluN2B
crystx
SeMet-1
GluN1a/
GluN2B
crystx
SeMet-2
GluN1a/
GluN2B
crystx
Ho3+
GluN1a/
GluN2B
crystx
Gd3+
Data collection
Beamline BL41XU 23ID-B/D 23ID-D 23ID-D 23ID-B 23ID-B
(Spring-8) (APS) (APS) (APS) (APS) (APS)
Space group P21 P21 P21 P21 P21 P21
Wavelength (Å) 1.0332 1.0332 0.9794 0.9794 1.5357 1.7111
Cell dimensions
a, b, c (Å) 118.6,
164.3,
163.2
116.8,
163.2,
163.1
118.6,
164.3,
163.8
118.7,
162.9,
163.4
119.4,
164.1,
163.9
119.7,
164.3,
164.1
β () 95.0 93.8 93.9 94.0 93.1 93.0
Resolution (Å) 50-5.7
(5.9)
50-3.95
(4.09)
50-6.0
(6.21)
50-4.8
(4.97)
50-7.5
(7.77)
50-7.8
(8.08)
Rmerge 0.1
(>1.0)
0.087
(>1.0)
0.078
(0.74)
0.077
(0.62)
0.09
(0.76)
0.082
(0.57)
I/σI 7.9 (1.4) 9.3 (1.02) 10.1 (1.6) 8.5 (1.3) 9.1 (1.2) 10.6 (1.6)
Completeness (%) 99.2 (100) 98.6 (99.4) 99.5 (97.4) 96.7 (98.3) 87.3 (99.5) 93.1 (98.5)
Redundancy 3.7 3.8 3.8 2.0 1.8 2.0
Refinement
Resolution (Å)
30.0-3.96
No. reflections
52,162
Rwork /Rfree 25.6/29.5
No. atoms
20,246
B-factors
202.8
R.m.s deviations
Bond lengths (Å) 0.002
Bond angles (º)
0.61
Ramachandran
statistics (%)*
Favored 92.1
Allowed 7.6
Highest resolution shell is shown in parenthesis. * Ramachandran statistics are calculated using Molprobity (47).
25
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